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首页> 外文期刊>Journal of bacteriology >Detection of growth sites in and protomer pools for the sheath of Methanospirillum hungatei GP1 by use of constituent organosulfur and immunogold labeling.
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Detection of growth sites in and protomer pools for the sheath of Methanospirillum hungatei GP1 by use of constituent organosulfur and immunogold labeling.

机译:通过使用成分有机硫和免疫金标记法检测饥饿甲基甲烷螺旋菌GP1鞘中的生长位点和原顶池。

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摘要

Methanospirillum hungatei GP1 integrated approximately 9% of cellular [35S]cysteine into its sheath. Autoradiography of sodium dodecyl sulfate-polyacrylamide gels revealed that [35S]cysteine was confined to the proteins released by the sodium dodecyl sulfate-beta-mercaptoethanol-EDTA solubilization method (G. Southam and T. J. Beveridge, J. Bacteriol. 173:6213-6222, 1991) and was not present in the proteins released by treatment with phenol (G. Southam and T. J. Beveridge, J. Bacteriol. 174:935-946, 1992). Limited labeling of exposed sulfhydryl groups on hoops produced from sheath material suggested that most organosulfur groups occur within hoops and therefore help contribute to resilience. Electron microscopic autoradiography demonstrated that sheath growth, which is most active at the sites of cell division (spacer region), occurs through the de novo development of hoops. For growth to occur in the spacer region, sheath precursors must transverse several periodic envelope layers, including the cell wall (a single layer) and the various lamellae of the spacer plug (T. J. Beveridge, G. D. Sprott, and P. Whippey, J. Bacteriol. 173:130-140, 1991).
机译:汉斯坦甲烷螺旋菌GP1将大约9%的细胞[35S]半胱氨酸整合到其鞘中。十二烷基硫酸钠-聚丙烯酰胺凝胶的放射自显影显示[35S]半胱氨酸仅限于十二烷基硫酸钠-β-巯基乙醇-EDTA溶解方法释放的蛋白质(G. Southam和TJ Beveridge,J. Bacteriol。173:6213-6222 ,1991)并且不存在于通过苯酚处理释放的蛋白质中(G.Southam和TJBeveridge,J.Bacteriol.174:935-946,1992)。由皮套材料制成的铁环上暴露的巯基基团的标记有限,这表明大多数有机硫基团都存在于铁环内,因此有助于提高弹性。电子显微放射自显影显示,鞘的生长在箍的从头发展,这是在细胞分裂部位(间隔区)最活跃的。为了使生长在间隔区中发生,外皮前体必须横穿几个周期性的包膜层,包括细胞壁(单层)和间隔塞的各种薄片(TJ Beveridge,GD Sprott和P. Whippey,J. Bacteriol) 173:130-140,1991)。

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